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通过肽核酸(PNA)杂交引导荧光微球共定位实现核酸的灵敏检测。

Sensitive detection of nucleic acids by PNA hybridization directed co-localization of fluorescent beads.

作者信息

Shiraishi Takehiko, Deborggraeve Stijn, Büscher Philippe, Nielsen Peter E

机构信息

Department of Cellular and Molecular Medicine; Faculty of Health Sciences; The Panum Institute; University of Copenhagen; Copenhagen N, Denmark.

出版信息

Artif DNA PNA XNA. 2011 Apr;2(2):60-66. doi: 10.4161/adna.2.2.16562.

Abstract

We have designed a pair of biotinylated peptide nucleic acid (PNA) probes targeting two sequences in 18S rRNA (from the parasite Trypanosoma brucei) at a distance of 191 nt (corresponding to maximum distance of ca. 60 nm) from each other. The PNA probes were individually bound to (strept)avidin-coated fluorescent beads, differing in size and color [green beads (1 µm) and red beads (5.9 µm)], thereby allowing distinct detection of each PNA probe by conventional fluorescence microscopy. These two PNA beads showed easily detectable co-localization when simultaneously hybridizing to a target nucleic acid. The assay detected the parasite 18S rRNA down to 1.6 fmol while there was no such co-localization visible with human 18S rRNA not containing the PNA targets. Furthermore, the assay showed positive detection with 1.6 ng of total RNA (corresponding to RNA from ca. 300 parasites). Upon further optimization this method may provide a new tool for a diagnosis of Human African Trypanosomiasis (HAT) and it may more generally have applications within diagnostics for (neglected) infectious diseases.

摘要

我们设计了一对生物素化的肽核酸(PNA)探针,靶向18S rRNA(来自寄生虫布氏锥虫)中的两个序列,彼此相距191个核苷酸(对应于约60纳米的最大距离)。PNA探针分别与大小和颜色不同的(链)霉抗生物素蛋白包被的荧光珠结合[绿色珠子(1微米)和红色珠子(5.9微米)],从而通过传统荧光显微镜对每个PNA探针进行清晰检测。当同时与靶核酸杂交时,这两个PNA珠显示出易于检测的共定位。该检测方法可检测低至1.6飞摩尔的寄生虫18S rRNA,而对于不含PNA靶标的人类18S rRNA则未观察到这种共定位。此外,该检测方法对1.6纳克总RNA(相当于约300个寄生虫的RNA)呈阳性检测。经过进一步优化,该方法可能为人类非洲锥虫病(HAT)的诊断提供一种新工具,并且更广泛地可能应用于(被忽视的)传染病诊断。

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